- Research article
- Open Access
- Open Peer Review
Clinical significance of serological biomarkers and neuropsychological performances in patients with temporal lobe epilepsy
© Chang et al; licensee BioMed Central Ltd. 2012
- Received: 2 October 2011
- Accepted: 14 March 2012
- Published: 14 March 2012
Temporal lobe epilepsy (TLE) is a common form of focal epilepsy. Serum biomarkers to predict cognitive performance in TLE patients without psychiatric comorbidities and the link with gray matter (GM) atrophy have not been fully explored.
Thirty-four patients with TLE and 34 sex - and age-matched controls were enrolled for standardized cognitive tests, neuroimaging studies as well as measurements of serum levels of heat shock protein 70 (HSP70), S100ß protein (S100ßP), neuronal specific enolase (NSE), plasma nuclear and mitochondrial DNA levels.
Compared with the controls, the patients with TLE had poorer cognitive performances and higher HSP70 and S100ßP levels (p < 0.01). The patients with higher frequencies of seizures had higher levels of HSP70, NSE and S100ßP (p < 0.01). Serum HSP70 level correlated positively with duration of epilepsy (σ = 0.413, p < 0.01), and inversely with memory scores in the late registration (σ = −0.276, p = 0.01) and early recall score (σ = −0.304, p = 0.007). Compared with the controls, gray matter atrophy in the hippocampal and parahippocampal areas, putamen, thalamus and supplementary motor areas were found in the patient group. The HSP70 levels showed an inverse correlation with hippocampal volume (R square = 0.22, p = 0.007) after controlling for the effect of age.
Our results suggest that serum biomarkers were predictive of higher frequencies of seizures in the TLE group. HSP70 may be considered to be a stress biomarker in patients with TLE in that it correlated inversely with memory scores and hippocampal volume. In addition, the symmetric extratemporal atrophic patterns may be related to damage of neuronal networks and epileptogenesis in TLE.
- Neuropsychological performances
- Temporal lobe epilepsy
- Gray matter atrophy
- Heat shock proteins
Temporal lobe epilepsy (TLE) represents the most common and likely to be medically refractory focal epilepsy in adults, with an estimated prevalence of 40% among epilepsy patients . Although epileptic focus in most cases of TLE originates from the temporal lobe and particularly the hippocampus, virtually all patients develop complex partial seizures with or without secondary generalization . Antiepileptic drugs (AEDs) are usually successful in controlling secondarily generalized seizures, however as many as 30% to 40% of TLE patients still have seizures despite receiving appropriate medical management . Those with pharmacoresistant TLE often require surgical treatment  along with lifelong AED therapy, and are associated with greater comorbidities and functional disabilities .
Proper selection of serological biomarkers, for example prolactin , can extend the diagnostic repertoire of epileptic seizures in the clinical setting. There were studies exploring the relationship between serum S100ß protein (S100ßP), neuron specific enolase (NSE) and heat shock protein 70 (HSP70) in Alzheimer dementia , status epilepticus  and epilepsy syndrome . Upregulation of HSP70 protects against intracellular amyloid toxicity by rescuing proteasomal activity . Pathology study in sudden and unexpected death in epilepsy suggested that HSP70 overexpression indicates acute neuronal injury occurring in the ante-mortem stage . Elevated serum NSE has been reported in patients with status epilepticus, complex partial status, in addition to TLE [8, 10, 11]. In TLE, a few studies have suggested that serum S100ßP [12, 13], NSE  or HSP70 [15–17] may be useful biomarkers for central nervous system damage. However, little data exists with regards to these biomarkers and cognitive performances in TLE. Elevation of plasma nuclear and mitochondrial DNA has been considered to be the consequence of neuronal cell death in the brain parenchyma, and has been linked with poor outcomes in bacterial meningitis and ischemic stroke [18, 19]. However, whether these two biomarkers are also associated with poor cognitive performances in TLE has not been reported before.
TLE can be a progressive disorder, potentially resulting in structural damage and a decline of cognitive abilities over time . Impairment in cognitive performance beyond the memory domain has been frequently reported in patients with TLE [21, 22], and a link between cognitive deficits with structural changes has been proposed. One meta-analysis reviewed the voxel-based morphometry (VBM) results in patients with TLE  and showed extratemporal gray matter (GM) atrophy. Although GM atrophy in TLE has been reported to be greater on the ipsilateral side in terms of epileptogenesis, the correlation accounting for cognitive deficits and the relationship with biomarkers have not been fully explored.
Recent studies have highlighted that self-propagating seizure activities in TLE may result in dysregulated inflammation, blood brain barrier damage and neuronal damage . Since HSP70, S100ßP, NSE, as well as plasma nuclear and mitochondrial DNA levels have been shown to reflect central nervous system damage, the present study hypothesized that these biomarkers may be of prognostic value in TLE patients from the cognitive aspect. We attempted to validate our hypothesis by measuring these biomarkers in TLE patients compared with age-and sex-matched controls, and compared the cognitive performances and structural imaging analysis using VBM in the GM areas. Furthermore, correlations between the biomarkers with duration of epilepsy, frequency of seizures and GM volume in the TLE group were examined in an attempt to understand the relationship between these biomarkers in predicting the severity of TLE and related neuronal damage.
This was a single center, age-and sex-matched cross-sectional study which was approved by the Institutional Review Board of Chang Gung Memorial Hospital and complied with the ethical standards established in the Declaration of Helsinki. The experiments were undertaken with the written, informed consent of each subject and their caregiver (when appropriate).
This study was initiated at the epilepsy outpatient clinic of Kaohsiung Chang Gung Memorial Hospital in 2009. Patients followed up as the epilepsy cohort  all underwent an extensive investigation including clinical history, comprehensive neurologic examination, interictal EEG and routine visual MRI analysis, the protocol of which included T1 and T2 sequences in axial and coronal planes.
The clinical diagnosis of TLE was based on the International League Against Epilepsy criteria (1997) as follows: (1) seizure semiology consistent with TLE, with abdominal, epigastric, psychic, or autonomic auras, followed by behavioral arrest, progressive alteration of consciousness, oroalimentary, and manual automatisms; (2) mesial and/or anterior temporal interictal spikes from video-electroencephalography (EEG) or bilateral sphenoidal EEG; and (3) no lesions other than increased T2 signal and/or atrophy in hippocampal formation identified by MRI.
Because it was not possible to combine all the influential factors in the TLE group to produce a uniform population, we only included non-surgical patients. By family history and past medical history review, none of our study patient had family trait or childhood febrile seizure history. Additional exclusion criteria in this study included a known history of mental retardation and a psychiatric comorbidity that prevented either a neuropsychiatric interview or neuroimaging. We also excluded patients with any of the following: (1) medication history of psychoactive or central nervous system depressant drugs; and (2) abnormal liver or renal functions. These exclusion criteria were added to avoid the confounding effects of medication and physical disorders on the cognitive test results.
After screening our TLE cohort , 34 patients (15 males and 19 females) fulfilled the inclusion and exclusion criteria, agreed to participate in the study, and completed it. Data for the age at onset, duration of epilepsy, average seizure frequency per month during the previous year, and numbers of AED were analyzed. According to the seizure frequency, patients with two or fewer seizures per month were classified as Group 1, and patients with more than two seizures per month as Group 2. Furthermore, 34 age-and sex-matched healthy subjects from the normative database were used as controls for the biomarkers, neuropsychological testing and MRI comparison. The age of each control subject was within 1 year of the matched TLE patient. None of the control subjects had a history of neurologic or neuropsychiatric disorders, and all had normal MRI and basic blood test results (liver and renal function tests, electrolytes, and complete blood cell counts).
Analysis of serological biomarkers
Blood samples were taken between 8 and 10 am after overnight fasting for the analysis of serum levels of HSP70, NSE and S100ßP. Liver and renal function tests, electrolytes, and complete blood cell counts were also analyzed by the central laboratory of Chang Gung Memorial Hospital-Kaohsiung.
For each patient, 5 ml of peripheral venous blood was collected into a serum separating tube. Plasma was prepared using EDTA-containing tubes and centrifugation at 3,000 rpm for 10 minutes, isolated, and immediately stored at −80 C in multiple aliquots. Serum HSP70, NSE and S100ßP levels were measured using an enzyme-linked immunosorbent assay (ELISA) kit (HSP70: EKS-750, Assay Design, San Francisco, CA, USA.; NSE: TM E-4700, Labor Diagnostika Nord, Nordhorn, Germany; S100ßP: RD192090100R, BioVendor, Brno, Czech Republic). In the ELISA, the samples were incubated in multiwell plates that had been coated with markers specific for anti-HSP70, anti-NSE, and anti-S100ßP antibodies. The ELISA procedures followed the manufacturer's protocols. The degrees of enzymatic turnover of the substrate were determined by dual wavelength absorbance measurements at 450 nm using a multiscan spectrum reader (Thermo Scientific, Miami, FL, USA). The antigen standards were used to plot a standard curve of absorbance versus antigen concentration from which the antigen concentrations in the unknowns were calculated.
Analysis of plasma nuclear and mitochondrial DNA levels
To evaluate the neuronal cell damage, we detected the released specific mitochondrial DNA (ND2 gene) and nuclear DNA (beta globulin gene) levels in plasma by real-time quantitative PCR methods [19, 26, 27]. The analysis of plasma nuclear and mitochondrial DNA levels followed our previous methods [18, 19]. In brief, 5 ml of peripheral venous blood in an EDTA-containing tube was collected and the blood sample was centrifuged at 3000 rpm for 10 minutes. 400 µl of plasma sample extracted by a QIAamp DNA Mini Blood Kit (No. 51304, Qiagen, Düsseldorf, Germany) was used for each measurement. Primers of the beta globulin gene (forward: 5'-GTG CAC CTG ACT CCT GAG GAG A-3'; reverse: 5'-CCT TGA TAC CAA CCT GCC CAG-3') and ND2 gene (forward: 5'-CAC AGA AGC TGC CAT CAA GTA-3'; reverse: 5'-CCG GAG AGT ATA TTG TTG AAG AG-3') were used, and the concentration adjusted to 10 µM containing 0.2 µl of each primer, 10 µl 2X SYBR Green PCR Fast Master Mix (No. 4385612, Applied Biosystems, San Francisco, CA, USA), 7.6 µl H2O and 2 µl plasma DNA sample. The mixture was placed in a StepOnePlus real-time PCR system (Applied Biosystems) for reaction following the standardized PCR procedure for 40 cycles: 95 C for 20 seconds, followed by 95 C for 3 seconds and 60 C for 30 seconds. Quantification of the PCR results followed the Pfaffl method.
Cognitive and behavior tests
All of the cognitive tests were performed during the interictal state as evidenced by the EEG recording before the cognitive test. A clinical neuropsychologist blinded to the patients' clinical diagnosis performed the neuropsychological tests which were chosen to assess memory, executive, attention, and visuospatial functions [29–31]. Verbal and visual episodic memory were assessed by a modified California Verbal Learning Test-Mental Status  and the Rey-Osterrieth Complex figure after a 10-minute delay. Language screening included the 16-item Boston Naming Test and 3-step comprehension and semantic verbal fluency.
Visuo-spatial abilities were assessed by a modified Rey-Osterrieth Complex Figure, pentagons, a transparent cube copy, and by the number location test from the Visual Object and Space Perception Battery. The ability to perform five arithmetic calculations was assessed, while frontal lobe function was assessed by digit forward and backward span, design fluency, Stroop Interference test, and the Modified Trails B test. Neuropsychiatric inventory (NPI) was used to assess behavioral symptoms. All of the tests were administered to both the patients and the controls for a statistical comparison of non-standardized tests.
MRI protocols and VBM
MRI was performed using a 3.0 Tesla scanner (Excite, GE Medical System, Milwaukee, WI, USA) equipped with echo-planar capability. Three-dimensional spoiled gradient-recalled acquisition in a steady state sequence was performed with the following parameters: TR/TI = 8600 ms/400 ms, FOV: 240 mm × 240 mm, slice thickness 1 mm.
VBM was processed using the SPM5 software package (http://www.fil.ion.ucl.ac.uk/spm) with study specific templates . All T1-weighted images were spatially normalized into the standardized Montreal Neurological Institute space using a 12-parameter affine transformation and non-linear normalization. The study-specific template was then smoothed with an 8 mm full-width at half-maximum (FWHM) isotropic Gaussian kernel.
The original images were warped to match the customized templates and re-sliced onto a voxel size of 1 × 1 × 1 mm to minimize partial volume effects. The images were segmented into gray, white, and cerebrospinal fluid (CSF) compartments with intensity inhomogeneity correction, modulated with Jacobian determinants to compensate for volume changes in non-linear spatial normalization, and smoothed with a 10 × 10 × 10 mm FWHM isotropic Gaussian Kernel . A general linear model was used to assess statistical differences in GM.
Categorical variables were compared using the chi-square test. Neuropsychiatric performances between the two groups were analyzed by the Mann-Whitney U test with Bonferroni correction. Partial correlation analysis between duration of epilepsy and serum biomarker/neuropsychological performances was performed with age being considered as a confounding factor. Multiple linear regression analysis was used to examine the relationship between GM atrophy and serum biomarkers levels. All statistical analyses were performed using the SAS software package (version 9.2, SAS Statistical Institute, Cary, NC, USA). A p value < 0.01 was considered statistically significant.
For VBM analysis, a significance threshold was set at p < 0.001 and corrected for multiple comparisons across the whole brain (false discovery rate) with an extended threshold of 250 voxels and applied to the resulting t-statistic maps of GM. To detect any correlation of clinical data with GM atrophy, partial correlation analysis of GM partitions was applied to the biomarkers adjusted for the effect of age at a significance of p < 0.01, corrected for multiple comparisons.
Demographic data and clinical characteristics of the patients with TLE
The age of the patient group was 37.1 ± 10.3 years, which was not significantly different from the control group (37.2 ± 10.2 years). Educational levels were not significantly different between the patient group (11.5 ± 4.3 years) and the controls (12.2 ± 3.4 years). The age of onset in the patient group was 18.8 ± 12.7 years and the duration of epilepsy was 18.9 ± 11.9 years. According to seizure frequency defined above, 22 patients were classified as Group 1 (0.8 ± 0.3 times per month), and 12 patients as Group 2 (3.3 ± 0.9 times per month). Eight patients received monotherapy, and the remaining 26 patients received polytherapy including 19 patients with two AEDs and 7 patients with 3 AEDs. Among the patients with epileptic focus, 21 had left temporal origins, and 13 from the right side. According to semiology, 9 patients experienced complex partial seizures only, while the other 25 patients had partial seizures with or without secondary generalization. Two patients had one or more seizures despite being treated with two consecutive first-line antiepileptic medications.
Biomarkers and cognitive tests
Biomarkers and neuropsychiatric performances between patients with temporal lobe
Controls (n = 34)
TLE patients (n = 34)
Heat shock protein 70 (μg/ml)
130.84 ± 61.1
194.5 ± 116.1**
Non-specific enolase (ng/ml)
9.43 ± 1.9
9.51 ± 1.9
S100ß protein (pg/ml)
70.52 ± 28.0
99.83 ± 45.7 **
Plasma nuclear DNA (ng/ml)
28.62 ± 2.5
29.19 ± 2.7
Plasma mitochondrial DNA (ng/ml)
21.33 ± 1.1
21.15 ± 1.0
Verbal Memory CVLT-MS (9)
6.18 ± 1.1
5.18 ± 1.5**
7.74 ± 1.1
7.36 ± 1.4
8.24 ± 0.9
8.06 ± 1.2
8.59 ± 0.7
8.15 ± 1.0
30 sec free recall
8.65 ± 0.7
7.67 ± 2.0**
10-min free recall
8.38 ± 1.2
7.18 ± 2.3**
8.53 ± 0.9
7.55 ± 1.8
Modified Rey-Osterrieth recall (17)
15 ± 2.5
11.64 ± 4.5**
Modified Rey-Osterrieth copy (17)
17 ± 0
16.79 ± 0.7
Cube copy (2)
1.82 ± 0.5
1.05 ± 0.9
Pentagon copy (1)
1 ± 0
0.82 ± 0.4
Visual object and space perception (10)
8.29 ± 2.0
8.64 ± 1.8
Speech and Language Ability
Semantic Fluency (1 minute)
21.59 ± 3.9
15.3 ± 5.4**
15.75 ± 2.8
11.54 ± 3.4**
13.83 ± 3.8
9.26 ± 2.1**
24.28 ± 6.2
16.82 ± 6.2**
Boston naming test (16)
15.58 ± 0.8
14.36 ± 2.2**
3.88 ± 0.3
3.51 ± 0.9
Abstract thinking (3)
2.58 ± 0.7
1.97 ± 1.2
Problem solving (3)
2.60 ± 0.7
2.00 ± 1.1
5.0 ± 1.6
Stroop interference correct (1 minute)
54.1 ± 10.9
40.33 ± 14.6**
10.78 ± 3.0
8.56 ± 5.6*
Trail Making test time (< 120 seconds)
23.6 ± 11.6
47.8 ± 35.3**
Correct line in Trail Making (14)
13.13 ± 2.7
11.92 ± 3.5
4.75 ± 0.7
4.51 ± 0.8
8.40 ± 0.8
7.44 ± 1.4**
Neuropsychiatric inventory score
1.91 ± 6.6
2.84 ± 5.5
In the selected cognitive tests, the short and long delayed verbal memory, visual memory, speech and language ability, executive function tests and digit forward spans were all significantly lower in the patient group than in the control group (all p < 0.01). There was no statistical difference in NPI total score between the patients and the controls.
Correlation study between biomarkers with cognitive tests
In the patient group, the correlation between age and duration of epilepsy was not significant (σ = 0.313, p = 0.07). Decreased memory scores in the CVLT-MS late registration (σ = −0.276, p = 0.01) and early recall score (σ = −0.304, p = 0.007) were inversely associated with serum HSP70 level. The level of plasma nuclear DNA showed an inverse correlation with verbal fluency (σ = −0.297, p = 0.008). A positive correlation was found between plasma nuclear DNA and Trail Making test completion time (σ = 0.333, p = 0.003), however after enrolling the duration of epilepsy as a covariate into the regression model, the correlation was not significant.
GM atrophy and regional variability
Voxel-based morphometry of gray matter atrophy analysis
Right inferior temporal
Right medial temporal
Right supplementary motor area
Left supplementary motor area
Right caudate nucleus
Clinical characteristics, biomarkers and neuropsychological tests results between Group 1 and 2
Relationship of clinical characteristics with biomarkers and neuropsychiatric performances in patients with temporal lobe epilepsy
Duration of epilepsy
Group 1 (n = 22)
Group 2 (n = 12)
Duration of epilepsy (years)
16.7 ± 8.5
20.3 ± 13.6
Number of antiepileptic drugs used Biomarkers
1.6 ± 0.6
2.52 ± 0.7
Heat shock protein 70 (µg/ml)
123.4 ± 34.7
324.7 ± 97.4**
Non-specific enolase (ng/ml)
8.4 ± 1.2
11.3 ± 1.13**
S100 ß protein (pg/ml)
79.04 ± 12.5
148.95 ± 43.6**
Plasma nuclear DNA (ng/ml)
29.22 ± 2.2
30.33 ± 2.2
Plasma mitochondrial DNA (ng/ml)
21.04 ± 1.0
21.13 ± 1.1
Verbal Memory CVLT-MS (9)
30 sec free recall
7.86 ± 1.5
7.27 ± 2.8
10-min free recall
7.23 ± 1.9
7.09 ± 2.9
7.50 ± 2.0
7.64 ± 1.6
Modified Rey-Osterrieth recall (17)
16.77 ± 0.8
16.82 ± 0.6
Cube copy (2)
0.91 ± 0.9
1.18 ± 0.9
Pentagon copy (1)
0.82 ± 0.4
0.82 ± 0.4
Semantic fluency animal (1 minute)
14.09 ± 4.5
17.73 ± 6.6
Boston naming test (16)
14.36 ± 2.3
14.18 ± 2.4
3.45 ± 0.9
3.45 ± 1.0
Abstract thinking (3)
1.95 ± 1.2
2.27 ± 1.2
Problem solving (3)
2.00 ± 1.0
2.00 ± 1.18
Stroop interference correct (1 minute)
39.82 ± 16.5
42.64 ± 12.4
7.68 ± 5.7
9.00 ± 5.8
Trail Making test time (< 120 seconds)
51.68 ± 38.8
45.18 ± 32.1
7.27 ± 1.5
7.73 ± 1.1
In neuropsychological performances, there were no significant differences between Group 1 and 2. However, with regards to the duration of epilepsy, an inverse correlation was found in pentagon copy and comprehension, while a positive correlation was found in Trail Making test completion time (p < 0.01).
The present study explored the clinical significance of serum biomarkers in relation to epileptic characteristics, cognitive performance and regions of GM atrophy patterns in patients with TLE. There were three major findings. First, the TLE group had higher serum levels of HSP70 and S100ßP and lower cognitive test scores compared with the controls. The serum levels of HSP70, NSE and S100ßP were significantly higher in the TLE patients defined by a higher seizure frequency (Group 2). Second, the inverse relationship between serum HSP70 levels with hippocampal GM partitions, memory dysfunction and duration of epilepsy suggest that HSP70 can be treated as a stress marker in TLE. Third, although the high variabilities in the hippocampal volume suggest the relatively lateralized nature of TLE, the homogenous atrophic patterns in regions beyond the epileptic origin (i.e. the supplementary motor area, thalamus and striatum) suggest more extensive structural damage in this epileptic disorder.
We found higher HSP70 levels in patients with TLE as compared with the controls. HSP70 belongs to the family of heat shock proteins that is involved in normal cellular homeostasis and survival by acting as a molecular chaperone . It is a constitutive protein which is expressed after cell stress . The role of HSP70 in patients with epilepsy is controversial. The induction of HSP70 in patients with TLE may reflect the stress condition conveyed by epileptic activities , however, a compensatory upregulation for neuroprotection has also been proposed . In an animal model, overexpression of HSP70 due to status epilepticus had a positive correlation with seizure intensity, suggesting the role of HSP70 in reflecting the severity of neuronal damage . Overexpression of HSP70 has similarly been observed in the hippocampal end folium neurons in patients with TLE, suggesting a correlation with the neuronal loss . Although HSP70 expression in epilepsy may suggest stress rather than neuroprotection , induction of HSP70 in protecting hippocampal neurodegeneration via modulating endogenous glutamate expression has also been observed . Therefore, the elevated serum levels of HSP70 can only be considered as a stress biomarker reflecting neuronal cell damage in the hippocampus, since an inverse relationship with memory test scores and hippocampal volume was found in addition to the elevation of HSP70 levels in patients with higher seizure frequencies and longer duration of epilepsy.
Another serum biomarker in this study showing a higher level in the patients with TLE as compared with the controls was S100ßP. The S100ßP homodimer is a neurite growth-promoting factor , and is widely used as a parameter for glial activation and blood brain barrier disruption . In human tissues from patients with TLE, overexpression of S100ßP from astrocytes without a concurrent increase in glia fibrillary acidic protein suggests the pathophysiology of astrocyte dysregulation in TLE . An elevated CSF level of S100ßP has been considered as a site-specific marker in patients with intractable TLE , also reflecting the severity of acute brain injury . A significant elevation of serum S100ßP levels has been reported recently in Han Chinese TLE patients as compared to healthy controls, with a higher level especially in female patients . Whether or not S100ßP is a suitable marker for epilepsy is still inconclusive. Some reports have indicated no differences in serum levels of S100ßP between patients with TLE and controls [11, 40, 41]. Taken together with the results of our study in that S100ßP was significantly higher in Group 2 patients, we suggest that the serum concentration of S100ßP could be another useful biomarker in patients with TLE for the evaluation of seizure activity.
The release of NSE from damaged neurons resulting from increased permeability of the blood brain barrier following seizure has been proposed as a possible mechanism . In contrast with the uncertainties of S100ßP in epilepsy , the serum level of NSE is considered to be a more reliable marker for reflecting a longer duration of partial epilepsy . Although elevated serum NSE levels have been frequently reported in patients with partial seizures or status epilepticus [11, 14], the relationship with TLE was not found in a literature search. We did not detect a significant difference in NSE level between the TLE group and controls, however we did find higher serum NSE levels in the patients with a higher seizure frequency. Nevertheless, its role in relation to cognitive performance was not established in the present study nor was the correlation with duration of epilepsy in TLE patients. Compared with HSP70, the elevated S100ßP and NSE levels found in this study could be regarded as indirect evidence for blood brain barrier disruption.
Relatively little is known about circulating plasma nuclear and mitochondrial DNA in neurological diseases, however, they are generally considered to be markers of cell death in the form of necrosis or apoptosis . The elevated plasma nuclear and mitochondrial DNA levels observed in critically ill patients  suggests a release of extracellular DNA from necrotic cells. Our study failed to detect differences either in plasma nuclear or mitochondrial DNA levels between the patients with TLE or controls. The inverse correlation of plasma nuclear DNA levels with executive function test may imply it is a neuronal damage marker, however further studies are needed to substantiate this explanation.
In TLE, there is a strong asymmetrical distribution of temporal lobe abnormalities with respect to epileptogenesis, particularly in the hippocampus and also to a lesser degree on the parahippocampal and entorhinal cortex . In the present study, patients with TLE showed high lateralization of the epileptic focus from the initial EEG recording with ipsilateral hippocampal atrophy based on the morphometric data extracted from the hippocampus. It is worth pointing out that the correlation study between morphometric data with biomarkers was based on a hierachical order. We did not perform the correlation voxel-wisely to avoid the possibility of type I errors.
In contrast, in the extratemporal regions including the thalamus, supplementary motor area and caudate nucleus, the GM atrophy was relatively symmetric suggestive of common pathways of epileptogenesis through these structures. This observation may suggest the importance of kindling effects from the epileptic focus that either deactivate the inhibitory or stimulate the excitatory pathways and induce progressive damage to the related neuronal networks .
Although the study sample was small, we did not pool the patients into one in terms of epileptic lateralization for VBM analysis since the GM of the right and left cerebral hemispheres is asymmetric in healthy subjects, likely reflecting underlying functional specificity. The pathologic contribution from epilepsy to this asymmetry is substantially greater than normal underlying asymmetry. Since the study results were used to correlate with cognitive performances rather than tracing the epileptigenesis circuit, a general GM atrophic pattern of these patients was presented.
There are several limitations to this study. First, the patients were only enrolled if they had not received an operation for TLE, and we only selected patients without a history of mental retardation or psychiatric comorbidity. Whether the results of this study can only be applied to this unique epilepsy syndrome or whether they can be applied to the general population of epilepsy patients still requires larger study cohorts for verification. Second, long term AED therapy has been shown to contribute to atherosclerosis and oxidative stress in epilepsy patients . As this study enrolled only a small number of patients and as the use of AEDs was not the same among all patients, the effects of the AEDs were therefore difficult to conclude. Different AEDs may have diverse impacts on the selected serum biomarkers levels included in this study. As such, interpretation of changes in biomarkers in the patients should be treated with great care. Lastly, the study design was mainly focused on the clinical parameters and neuroimaging findings with relation to the serum biomarkers during the interictal state. Therefore, the observations here can not represent the ictal pathogenesis of this disease model in relation with these biomarkers.
The findings in the present study validated our initial hypothesis that biomarkers in the circulation may show predictive roles in the neuropsychological performance and neuroimaging changes in TLE. Serum levels of HSP70 had a positive correlation with the duration of epilepsy, hippocampal atrophy and memory dysfunction, suggesting that it can be used as a biomarker for stress-related neuronal damage. Moreover, compared with HSP70, the elevated S100ßP and NSE levels found in the present study may be regarded as indirect evidence for epileptic neuronal damage and blood brain barrier disruption. We are aware that the duration of epilepsy has been regarded as an important factor leading to the worsening of cognitive performance in patients with TLE  and this was also shown in the study results. The concurrent frontal-subcortical GM atrophy in patients with TLE reinforces the notion of a kindling phenomenon with neuronal damage from the related temporal foci in this highly lateralized epileptic disorder. A longitudinal study might extend the repertoire for disease progression while the evaluation in association with physiological parameters may unreveal the mechanism of epileptogenesis.
The authors wish to thank the patients and their caregivers for their time and commitment to this research. This study was supported in part by research grants NSC99-2314-B-182A-054-MY3 to C.C.C. and 99-2321-B-182A-002 to Y.C.C. from the National Science Council, Taiwan.
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